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高活性莫氏耶尔森菌植酸酶的定向进化

Directed evolution of a highly active Yersinia mollaretii phytase.

作者信息

Shivange Amol V, Serwe Annegret, Dennig Alexander, Roccatano Danilo, Haefner Stefan, Schwaneberg Ulrich

机构信息

Lehrstuhl für Biotechnologie, RWTH Aachen University, Worringerweg 1, Aachen, Germany.

出版信息

Appl Microbiol Biotechnol. 2012 Jul;95(2):405-18. doi: 10.1007/s00253-011-3756-7. Epub 2011 Dec 11.

Abstract

Phytase improves as a feed supplement the nutritional quality of phytate-rich diets (e.g., cereal grains, legumes, and oilseeds) by hydrolyzing indigestible phytate (myo-inositol 1,2,3,4,5,6-hexakis dihydrogen phosphate) and increasing abdominal absorption of inorganic phosphates, minerals, and trace elements. Directed phytase evolution was reported for improving industrial relevant properties such as thermostability (pelleting process) or activity. In this study, we report the cloning, characterization, and directed evolution of the Yersinia mollaretii phytase (Ymphytase). Ymphytase has a tetrameric structure with positive cooperativity (Hill coefficient was 2.3) and a specific activity of 1,073 U/mg which is ∼10 times higher than widely used fungal phytases. High-throughput prescreening methods using filter papers or 384-well microtiter plates were developed. Precise subsequent screening for thermostable and active phytase variants was performed by combining absorbance and fluorescence-based detection system in 96-well microtiter plates. Directed evolution yielded after mutant library generation (SeSaM method) and two-step screening (in total ∼8,400 clones) a phytase variant with ∼20% improved thermostability (58°C for 20 min; residual activity wild type ∼34%; variant ∼53%) and increased melting temperature (1.5°C) with a slight loss of specific activity (993 U/mg).

摘要

植酸酶作为一种饲料添加剂,通过水解难以消化的植酸盐(肌醇1,2,3,4,5,6 - 六磷酸)并增加无机磷酸盐、矿物质和微量元素在肠道的吸收,从而提高富含植酸盐的日粮(如谷物、豆类和油籽)的营养质量。已有报道通过定向进化来改善植酸酶的工业相关特性,如热稳定性(制粒过程)或活性。在本研究中,我们报道了耶尔森氏菌植酸酶(Ymphytase)的克隆、表征及定向进化。Ymphytase具有正协同性的四聚体结构(希尔系数为2.3),比活为1073 U/mg,约为广泛使用的真菌植酸酶的10倍。我们开发了使用滤纸或384孔微量滴定板的高通量预筛选方法。通过在96孔微量滴定板中结合吸光度和基于荧光的检测系统,对热稳定且有活性的植酸酶变体进行精确的后续筛选。在生成突变文库(SeSaM方法)和两步筛选(总共约8400个克隆)后,定向进化得到了一种植酸酶变体,其热稳定性提高了约20%(58°C处理20分钟;野生型残留活性约为34%;变体约为53%),解链温度升高了1.5°C,比活略有下降(993 U/mg)。

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